Process for selectively isolating IgY antibodies from egg yolk of an anseriform bird and IgY antibodies obtained thereby

ABSTRACT

The present invention mainly relates to a process for isolation and purification of yolk antibodies from egg yolk of an anseriform bird by an adsorption chromatographic procedure using a water insoluble non-charged absorbent to accomplish a desired separation of yolk antibodies, and by a salting-out procedure that differentially precipitates the IgY antibodies. The present invention also relates to the yolk antibodies produced thereby and various uses of such yolk antibodies.

RELATED APPLICATIONS

[0001] This application is a continuation-in-part and claims priority to U.S. application Ser. No. 09/733,210, filed Dec. 8, 2000, the content of which is incorporated herein by reference.

BACKGROUND OF THE INVENTION

[0002] 1. Field of the Invention

[0003] The present invention relates to a process for rapid isolation and purification of yolk antibodies, in particular IgY antibody, from anseriform bird yolk, and the yolk antibodies obtained thereby. More particularly, the present invention relates to a process for isolation and purification of yolk antibodies from anseriform bird yolk by an adsorption chromatographic procedure using a water insoluble non-charged absorbent to accomplish a desired separation of yolk antibodies, and by a salting-out procedure that differentially precipitates the IgY antibodies. The present invention also relates to uses of the IgY antibodies in quantitative or qualitative immunoassay or in the preparation of pharmaceutical compositions directing to an etiological agent of interest.

[0004] 2. Description of the Related Art

[0005] Antibodies are used widely in many biological investigations and clinical applications. Sera obtained from hyperimmunized mammalians are the most common source of polyclonal antibodies. Antibodies derived from such immune sera belong to a group of proteins called “immunoglobulins,” among which the immunoglobulin G (IgG) is the most abundant. The IgG molecule consists of three domains, namely two Fab regions and one Fc region. The Fab portion involves mainly in antigen binding. The Fc portion, though having no ability to bind with an antigen, directs several biological activity of an antibody, such as complement fixing and Fc receptor binding.

[0006] In the art of immunodiagnostics, an intact IgG molecule is not suitable for use in detection systems and immunological assays involving mammalian sera since the Fc region on an IgG molecule is capable of binding to Fc receptors, activating the complement system, and reacting with rheumatoid factor in mammalian sera. Removal of the Fc portion of an IgG molecule frequently leads to a reduction in the interference (E. Lamoyi, Methods in Enzymology 121:652-663, 1986).

[0007] Some of the suggested uses of antibody in immunotherapy include treating patients with intoxicated bacterial toxins or snake venoms (see, for example, U.S. Pat. No. 5,340,923 and U.S. Pat. No. 5,601,823), and protection of neonatal piglets against fatal enteric colibacillosis (see, for example, H. Brussow et al., J. Clin. Microbiol. 25:982, 1987; and C. O. Tacket et al., New Eng. J Med. 318:1240, 1988). Since the Fc fragment of an antibody molecule is known to be the most antigenic portion of the immunoglobulin (E. M. Akita et al., J. Immunol Methods. 162:155-164, 1993), cleavage of the same which results in the formation of an F(ab′)₂ fragment will reduce significantly a number of potential allergenic sites on the immunoglobulin molecule and is thus beneficial to human or an animal administered with the immunoglobulin.

[0008] Recently, the divalent F(ab′)₂ antibody fragment has been shown to be more useful in the immunodiagnostic tests (M. Muratsugu et al., J. Colloid Interface Sci 147:378, 1991); and J. L. Ortega-Vinuesa et al., J. Immunol Methods 90:29, 1996) and more suitable for development of the immunoassays involving mammalian sera than the parent IgG.

[0009] The F(ab′)₂ antibody fragment, however, has not found widespread use in clinical immunodiagnostic kits as one might expect. This may be attributed to the difficulties and cost-ineffectiveness of large scale production of the F(ab′)₂ fragments, which is conventionally made by pepsin digestion of IgG and subsequent purification via chromatography.

[0010] Ducks and their phylogenetically close relatives and some reptiles, such as turtles, have three kinds of serum immunoglobulins: a macromolecular immunoglobulin IgM (800 kDa in duck), and two isoforms of low molecular weight IgG with sedimentation coefficients of 7.8 S (in duck, 180 kDa) and 5.7 S (in duck, 130 kDa), respectively. (E. R. Unanue et al., J. Exp. Med. 121:697-714, 1965; H. M. Grey, J. Immunol 98:811-819, 1967); and B. Zimmerman et al., Biochemistry 10:482-448, 1971). Avian IgG is oftentimes called IgY due to their existence in egg yolk besides in sera. The 5.7 S IgY, constituted with shorter heavy chains, is structurally and antigenically similar to the F(ab′)₂ fragment of the 7.8 S IgY (FIG. 1), and this fact leads to the nomenclature of IgY (equivalent to 7.8 S IgY) and IgY(ΔFc) (equivalent to 5.7 S IgY) to represent both isoforms of IgY (K. E. Magor et al., J. Immunol. 149:2627-2633, 1992).

[0011] Studies conducted in the infected or experimentally immunized birds showed that duck antibodies are deficient in a number of biological effector functions, including complement fixation and Fe receptors binding, without sacrificing their binding activity to corresponding antigens (G. W. Litman et al., Immunochemistry 10:323, 1973; and T. E. Toth et al., Avian Dis. 25:17-28, 1981). This may reasonably result from the absence of an Fc-equivalent region of the IgY(ΔFc) antibody that constitutes the quantitatively major component of anseriform bird antibody response. It is thus believed that the IgY(ΔFc) antibody, which appears to be a structural and functional analog of the F(ab′)₂ fragment, would provide magnificent advantages in immunological uses, if a promising process for manufacturing the antibody could be found, and the appropriate physical requirements for its activity could be identified.

[0012] Avian yolk antibodies have been reported to exhibit useful properties for both research and clinical applications as mammalian antibodies do (see, for example, U.S. Pat. No. 5,340,923; U.S. Pat. No. 5,585,098; U.S. Pat. No. 5,601,823; and U.S. Pat. No. 5,976,519). Egg yolks derived from a laying hen is inexpensive and more convenient and safer to handle as compared to the hyperimmunized mammalian sera. More importantly, yolk antibodies are able to stand up to the scrutiny under modem animal protection regulations (A. Poison et al., Immunol. Commun. 9:475, 1980; and B. Gottstein et al.). These facts suggest a potential use of egg yolk as a commercial source of antibodies.

[0013] However, high contents of lipidic substances, such as fatty acids, cholesterol and lecithin, in egg yolk make the isolation of yolk antibodies a cumbersome and laborious task. Many efforts have been made in this regard. For instance, water soluble precipitants, including agar, pectin (Japanese Kokai No. 64-38098 published in Feb. 8, 1989), dextran sulfate (J. C. Jensenius et al., J. Immunol. Methods 46:63, 1981), natural gums (H. Hatta et al., J. Food Science 53:425, 1988) and polyethylene glycol (PEG) (A. Poison et al., Immunol. Invest. 14:323, 1985; see also U.S. Pat. No. 4,550,019 issued to A. Poison) were used to precipitate non-aqueous bio-molecules, mainly lipids and yolk granules, to thereby harvest a water soluble phase containing abundant yolk antibodies of the entire population. A. Hassl et al. developed a two-step chromatographic process, comprised of hydrophobic interaction chromatography and size exclusive chromatography, for further isolation of yolk antibodies of the entire population from a PEG-purified fraction (A. Hassl and H Aspock, J. Immunol. Methods 110:225, 1988). Akita et al. described an improved method for isolating IgY, in which yolk antibodies were extracted from chick eggs by diluting the egg yolks with a large volume of water and subjecting the resultant supernatant to size exclusive chromatography and/or ion exchange chromatography (E. M. Akita et al., J. Immunol. Methods. 160:207, 1993; and E. M. Akita and S. Nakai, J. Food Sci. 57:629, 1993).

[0014] However, all these studies and patents focus on the isolation of the entire population of yolk antibodies (which at least includes IgY present or absent Fc region) from avian eggs, rather than on the purification of IgY(ΔFc) and IgY antibodies selectively. Moreover, since IgY(ΔFc) antibodies are present only in birds belonging to the Order Anseriformes, including duck and goose, and since the lipid content in the egg yolk of the anseriform birds is reported higher than that in the galliform birds, such as chicken and turkey, the conventional methods described above provide no suggestion of a successful purification of IgY(ΔFc) antibody. IgY(ΔFc) antibody was only purified by co-precipitating with IgY from duck serum (D. A. Higgins et al., Veterinary Immunology and Immunopathology 41:169-180, 1995) with complexes and expensive procedures, but still no IgY(ΔFc) antibody alone was selected isolated from egg yolk.

[0015] Therefore, there exists a need for a rapid, cost-effective and high-throughput process that provides easy isolation of the desired yolk antibody (e.g., IgY(ΔFc)) from the antibody pool of anseriform bird egg while maintaining the activity of the antibody. The substantially purified IgY(ΔFc) antibody may acts as a new type of F(ab′)₂ antibody for various immunodiagnostic and immunotherapeutic uses.

SUMMARY OF THE INVENTION

[0016] Extensive research has been conducted to fulfill the industrial requirements for yolk antibodies as indicated above. It is unexpectedly found that a successful isolation of yolk antibodies from egg yolks of an anseriform bird can be readily accomplished through an adsorption chromatographic procedure using a water insoluble non-charged absorbent, and/or through a simple salting-out procedure that differentiates different isoforms of the yolk antibodies. According to the process of the present invention, the highly purified yolk antibodies, in particular the highly purified IgY(ΔFc), can be easily obtained with high yield in an economic manner, and are ready for a wide variety of immunological uses.

[0017] Accordingly, an object of the present invention is to provide a process for selectively isolating IgY antibodies from egg yolk of an anseriform bird, which is characterized in:

[0018] (a) absorbing yolk antibodies in a water-miscible fraction obtained from the egg yolk of an anseriform bird with a water insoluble non-charged absorbent selected from the group consisting of silicate, silicon compounds, carbonate, sulfate, phosphate, carbon, cellulose and synthetic fiber, ceramics, and metal oxide, and wherein the water insoluble non-charged absorbent is at an amount effective for separating the yolk antibodies from the water-miscible fraction; and

[0019] (b) flowing the water insoluble non-charge absorbent with a buffer to obtain an aqueous fraction containing the yolk antibodies.

[0020] In one embodiment, the water insoluble non-charged absorbent absorbs both the yolk antibodies and the majority of the water-miscible lipidic substances remaining in the water-miscible fraction. In another embodiment, the absorbent absorbs the water-miscible lipid substances, but does not substantially absorb the yolk antibodies (e.g., absorbs less than 40, 30, 20, or 10% of the yolk antibodies.

[0021] Another aspect of the invention is to provide a process for selectively isolating IgY antibodies from egg yolk of an anseriform bird, which is characterized in performing first salting out by salting out an aqueous fraction containing yolk antibodies with (NH₄)₂SO₄ of a first concentration ranging from about 15% (w/v) to about 24% (w/v), and wherein preferably not more than about 21% (w/v) based on the volume of the aqueous fraction, and then performing second salting out by salting out the aqueous fraction containing yolk antibodies treated in the first salting out with (NH₄)₂SO₄ of a second concentration ranging from about 25% (w/v) to about 40% (w/v), and wherein preferably not more than about 31% (w/v) based on the volume of the aqueous fraction treated in the first salting out.

[0022] Still another aspect of the invention is to provide a process for selectively isolating IgY antibodies from egg yolk of an anseriform bird, which is characterized in:

[0023] (a) absorbing yolk antibodies in a water-miscible fraction obtained from the egg yolk of an anseriform bird with a water insoluble non-charged absorbent selected from the group consisting of silicate, silicon compounds, carbonate, sulfate, phosphate, carbon, cellulose and synthetic fiber, ceramics, and metal oxide, and wherein the water insoluble non-charged absorbent is at an amount effective for separating the yolk antibodies from the water-miscible fraction;

[0024] (b) flowing the water insoluble non-charged absorbent with a buffer to obtain an aqueous fraction containing the yolk antibodies;

[0025] (c) salting out the aqueous fraction containing yolk antibodies in step (b) with (NH₄)₂SO₄ of a first concentration ranging from about 15% (w/v) to about 24% (w/v), and wherein preferably not more than about 21% (w/v) based on the volume of the aqueous fraction; and

[0026] (d) salting out the aqueous fraction containing yolk antibodies treated in step (c) with (NH₄)₂SO₄ of a second concentration ranging from about 25% (w/v) to about 40% (w/v), and wherein preferably not more than about 31% (w/v) based on the volume of the aqueous fraction treated in step (c).

[0027] According to the process of this invention, an abundant amount of a selected isoform of yolk antibodies, in particular IgY(ΔFc) antibody, available for various industrial applications can be obtained in an economic, efficient and time-saving manner.

[0028] It is still another object of the invention to provide the clinical and research uses of the IgY antibody so produced. In addition to the cost-effectiveness and ease of preparation, the IgY(ΔFc) antibody according to the present invention has advantages of being inactive to the complement system and rheumatoid factors in mammalian sera, and having poor cross-reactivity to mammalian IgG, and is thus particularly suitable for use in immunological assays involving mammalian sera with minimal interference. It would be appreciated by those skilled in the art that the IgY antibody can be present in the form of a single reagent for clinical, research and other applications, or included in a commercial kit as an active component.

[0029] It is another specific object of the invention to provide a reagent for immunoassay of an etiological agent of interest, comprising an IgY antibody obtained by the process according to this invention.

[0030] In many implementations, the methods enable the IgY(ΔFc) isoform (5.7 S) to be separated from other isoforms, e.g., the 7.8 S isoforms. In some implementations, the IgY(ΔFc) species (5.7 S) is at least 70, 80, 90, or 95% pure (w/v). It can be enriched at least 10, 20, 30, or 40 fold relative to the 7.8 S isoform. The highly purified yolk antibodies, in particular the highly purified IgY(ΔFc), can be obtained with high yield in an economic manner, and are ready for a wide variety of uses.

BRIEF DESCRIPTION OF THE DRAWINGS

[0031] The above and other objects and features of the present invention will become apparent with reference to the following description of the preferred embodiments taken in conjunction with the accompanying drawings, in which:

[0032]FIG. 1 illustrates a SDS-PAGE analysis comparing the antibody capturing abilities of four absorbents: lane 1, the partially purified antibody extract; lane 2, the solution flowing through 2% fumed silica; lane 3, the solution flowing through 3% silica dioxide; lane 4, the solution flowing through 3% Celite diatomite; lane 5, the solution flowing through 3% Celite diatomite hyflo-Cel; and lane 6, the solution flowing through 5% Celite diatomite hyflo-Cel;

[0033]FIG. 2 illustrates the electrophoresis results of the purified yolk antibodies using fumed silica as the absorbent run on an 8% SDS-polyacrylamide gel: lane 1, the partially purified antibody extract; lane 2, the solution flowing through 2% fumed silica; lane 3, the eluate from the fumed silica pellet; lane 4, the antibody product precipitated with 21% (w/v) ammonium sulfate in the first precipitation step; and lane 5, the antibody product precipitated with 31% (w/v) ammonium sulfate in the second precipitation step;

[0034]FIG. 3 illustrates the electrophoresis results of the purified yolk antibodies using Celite diatomite as the absorbent run on an 8% SDS-polyacrylamide gel: lane 1, the partially purified antibody extract; lane 2, Celite diatomite filtrate; lane 3, the antibody product precipitated with 21% (w/v) ammonium sulfate in the first precipitation step; lane 4, the antibody product precipitated with 31% (w/v) ammonium sulfate in the second precipitation step; and lane 5, the antibody product precipitated with 16% (w/v) sodium sulfate in the second precipitation step; and

[0035]FIG. 4 illustrates the electrophoresis results of the purified yolk antibodies using fumed silica as the absorbent run on an 8% SDS-polyacrylamide gel: M, molecular weight marker; lane 1, the partially purified antibody extract; lane 2, the solution flowing through 2% fumed silica; lane 3, the eluate from the fumed silica pellet; lane 4, the antibody product precipitated with 21% (w/v) ammonium sulfate; and lane 5, the antibody product purified by affinity chromatography.

DETAILED DESCRIPTION OF THE INVENTION

[0036] The yolk antibodies are abundant in the bird serum and the eggs laid by the bird. However, as described above, collection of the antibody from the egg is usually preferred on account of the cost. The laying hen transfers both of the IgY and IgY(ΔFc) isoforms from serum to the egg yolk. In principle, each duck egg contains about 1 to about 4 mg IgY/ml and about 3 to about 12 mg IgY(A Fc)/ml in the yolk and, therefore, the total quantity of the antibodies contained in a single egg is estimated to be 15 to 80 mg of IgY and 45 to 240 mg of IgY(ΔFc). The large volume of egg yolk produced vastly exceeds the volume of the serum that can be safely obtained from the birds over any given time period. In addition, extraction of yolk antibodies can be performed on a large scale without costly investment. Preferably, antibodies in the present invention are obtained from eggs of an anseriform bird immunized with a specific antigen.

[0037] In accordance with the present invention, it provides a process for efficiently isolating antibodies from egg yolk, in which the so-called “adsorption chromatography” or “differential salting-out,” which may be used alone or in combination with the other, acting as critical steps in the isolation.

[0038] As used herein, the term “adsorption chromatography” is directed to a type of separation method involving the use of a stationary phase to selectively take up and concentrate the desired solutes from a mobile phase. According to one aspect of the present invention, a water insoluble non-charged absorbent acts as the active constituent in the stationary phase to separate the yolk antibodies by adsorbing the yolk antibodies in the water insoluble non-charged absorbent and also trapping water-miscible lipidic impurities that are normally present in egg yolk.

[0039] In a preferred embodiment of the present invention, the yolk is firstly separated from the egg white, and then washed with distilled water to remove as much albumen as possible. The vitelline membrane encapsulating the yolk is punctured, and the separated yolk fraction is then diluted with an effective amount of an aqueous buffer or water to form a suspension of the egg yolk. Preferably, the collected egg yolk is diluted with an aqueous buffer solution or distilled water ranging from about 2 parts to about 40 parts by volume, more preferably from about 5 parts to about 30 parts by volume, per 1 part of the egg yolk. Value of pH may be an important factor during the stage of partial purification (E. M. Akita and S. Nakai, J. Food Sci. 57:629, 1993), at least in some implementations. For the best recovery of yolk antibodies, pH is preferably set within a range of about 5 to about 7. Desirably, the temperature in this step is within a range of about 0° C. to about 60° C. The suspension of the egg yolk is gently agitated to form a homogenous mixture, and then allowed to stand for a period of time sufficient to form the aqueous and non-aqueous phases. The water insoluble materials, including non-aqueous bio-molecules such as lipoproteins, phospholipids, sterols and the like, are then removed from the aqueous yolk suspension by centrifugation. The resulting antibody-containing supernatant may then be separated from the viscous precipitant by decanting, suctioning, or other like methods known in the art.

[0040] In general, the lipid content of the water-miscible fraction thus obtained is still so high as to be adverse to the subsequent manipulation. According to the present invention, a stationary phase containing a water insoluble non-charged absorbent is incubated with the water-miscible fraction in a sufficient amount to absorb the yolk antibodies and to adsorb the majority of the water-miscible lipidic substances remaining in the water-miscible fraction. The suitable absorbents include but are not limited to silicate, silicon compound, carbonate, sulfate, phosphate, carbon, cellulose and synthetic fiber, ceramics, and metal oxide, and wherein the silicate includes synthetic or natural clays, kaolin, talc, and calcium silicate; the silicon compound includes fumed silica, amorphous silica, silica dioxide, silica gel, silicates, diatomaceous earth, and Fuller's earth; carbonate includes calcium carbonate and barium carbonate; sulfate includes calcium sulfate; phosphate includes calcium phosphate; carbon includes activated carbon and carbon fiber, cellulose and synthetic fiber includes cellulose powder; ceramics includes porosity ceramics; and metal oxide includes aluminum oxide and titanium oxide. Particularly preferred absorbents are fumed silica, silica dioxide and diatomaceous earth. The working ratio of the absorbent to the water-miscible fraction can vary over a wide range depending upon the properties of the absorbent chosen. When fumed silica is used in this process, it is preferably added to a concentration of equal to or higher than about 0.1% by weight, and more preferably ranged between about 0.3 to about 5.0% by weight, based on the volume of the water-miscible fraction to be treated. When the absorbent is silica dioxide or diatomaceous earth, the adsorption chromatography according to this invention is preferably carried out at more than about 1% by weight, and more preferably in a range of about 3 to about 20% by weight, of the absorbent based on the volume of the water-miscible fraction to be treated.

[0041] The adsorption chromatography according to this invention can be effectuated by any conventional ways, such as batch treatment of the water-miscible fraction with an absorbent or flowing the water-miscible fraction over a chromatography column packed with the absorbent, as long as the amount of the yolk antibodies retained on the surfaces of the absorbent is satisfactory. The reaction time and temperature during the treatment are not critical to the results, and a reaction temperature of about 4 to about 30° C. and a reaction time of about 10 to about 60 minutes are usually feasible. While the adsorption procedure can be repeated several times, each with fresh absorbent, if necessary, a single operation is normally sufficient. By way of this procedure, the lipids and most of the non-lipid substances can be successfully separated into two immiscible phases while yolk antibodies can also be absorbed.

[0042] Depending upon the capability of the selected absorbent to capture immunoglobulins, the yolk antibodies can be recovered from either an eluate eluted from the stationary phase or the “flow-through solution” which, as used herein, is intended to represent the solution passing through the stationary phase. As shown in the preferred embodiments given in the text, the yolk antibodies are mainly present in the stationary phase when fumed silica or silica dioxide is used as the absorbent, whereas diatomaceous earth leaves more than about 60% of the antibodies in the flow-through solution.

[0043] The choice of a particular method to obtain yolk antibodies can be determined by the skilled artisan. Typically, the yolk antibodies are obtained in an aqueous fraction by flowing the water insoluble non-charged absorbent with a buffer, and wherein the buffer is at a pH of lower than about 4 or higher than about 8 or containing a chaotropic agent can be utilized in the present invention to obtain the yolk antibodies from the stationary phase without substantially dissociating the lipidic substances from the stationary phase, such that an antibody-containing eluate is formed. As used herein, the term “eluate” is directed to a solution containing the desired substances unbound by the eluent from the stationary phase. The term “chaotropic agent” or “chaotrope” is directed to a chemical capable of inducing a conformational change in a protein molecule, such as an antibody molecule, which is therefore often known as a protein denaturant. According to the invention, most of the bound antibodies can be successfully eluted with any neutral buffer containing moderate concentration (>1 M) of a chaotropic agent. In most instances, removal of the chaotrope after elution will restore the native protein structure.

[0044] The useful buffer include but are not limited to 0.1 M glycine-HCl, pH 2.3; 0.1 M glycine-HCl, pH 10.0; 3M to 8 M guanidine-HCl (e.g., 3 to 6M), pH 3.0; 3.0 M potassium chloride; 5 M potassium iodide; 3.5 M magnesium chloride; 1-3 M ammonium/sodium/potassium thiocyanate (or e.g., at least 1M) and 6 M urea (or e.g., at least 4, 5, or 6M urea). With respect to the activity of the recovered antibodies, however, a moderate-ionic strength, chaotrope-containing, neutral pH buffer, such as 3 M sodium thiocyanate buffered in 20 mM MES buffer (pH 5.8) or 20 mM Tris(hydroxymethyl)-aminomethane (pH 7.5), is more suitable for practicing the invention. The active state of the collected antibodies can be easily restored by, for example, extensive dialysis against a low-ionic strength, non-chaotrope-containing, and weakly acidic buffer.

[0045] According to one aspect of the present invention, the aqueous fraction including the eluate or the flow-through solution, which is enriched with antibodies, can subsequently be subjected to a procedure of differential salting-out to separate yolk antibody isoforms.

[0046] The term “salting-out” as used herein takes on its common meaning in the art of protein chemistry and is directed to the addition of a non-denaturing salt or salts to a mixture or production batch to decrease the solubility of proteins, which leads to the precipitation or coagulation of the proteins. By the term “differential salting-out” is meant a salting-out process that differentially precipitates or coagulates two or more proteins from a mixture by varying the concentration of the added salt or salts. In the present invention, the proteins intended to be differentially precipitated are the isoforms of yolk antibodies, i.e., IgY and IgY(ΔFc). Examples of the non-denaturing salts useful for precipitation of the yolk antibodies include but are not limited to NaCl, Na₂SO₄, (NH₄)₂SO₄, KCl, CaCl₂, and MgSO₄. Preferably, the non-denaturing salt is Na₂SO₄ or (NH₄)₂SO₄, and (NH₄)₂SO₄ is the most preferred. The salt concentration for differentially precipitating yolk antibody isoforms depends on the type of the salt and can be determined by a skilled artisan through simple tests. According to a preferred embodiment of the present invention, in which (NH₄)₂SO₄ is employed, IgY is firstly salted out at a concentration ranging from about 15% (w/v) to about 24% (w/v), and wherein preferably is equal to or lower than about 21% (w/v), of the salt on the basis of the treated volume of the aqueous fraction, while IgY(ΔFc) is precipitated as the concentration of the salt ranging from about 25% (w/v) to about 40% (w/v), and wherein preferably is about 31% (w/v) based on the treated volume of the aqueous fraction. It should be appreciated that the sequence of precipitation of the two antibody isoforms could be also variable depending on the salt chosen. The combined use of two or more salts in this procedure, e.g., firstly precipitating a first isoform with one salt followed by precipitating a second isoform with another salt, is also feasible. The differential salting-out procedure according to the present invention dramatically accomplishes a main object of the present invention, i.e., essential selectively separation of the desired IgY comprising IgY and IgY(ΔFc) antibodies from the whole population of yolk antibodies constituted by both IgY and IgY(ΔFc).

[0047] If obtaining the antibodies with a higher purity is desired, the precipitated antibodies can be re-dissolved in a suitable buffer system and subjected to additional purification procedures, such as size exclusive chromatography, hydrophobic interaction chromatography, ion-exchange chromatography and immuno-affinity chromatography.

[0048] As used herein, the term “immunoaffinity purification” or “immunoaffinity chromatography” is directed to a type of separation method based on the binding characteristics of antibodies for a specific antigen. That is, the antibodies that bind to a specific antigen under a particular condition are separated from the unbound antibodies under that condition. The present invention contemplates the use of immunoaffinity purification to eliminate irrelevant proteins, in particular the non-antigen-binding immunoglobulin.

[0049] According to the present invention, the immunoaffinity purification is conducted by use of an “antigen matrix” comprised of antigen immobilized onto an insoluble support. The type of the support is not critical to the immunoaffinity purification of the invention. Any conventional support material suitable for the covalent attachment of an antigen and inert to the interaction between the desired antibody and the antigen immobilized thereon is useful. Usually, the support is made of crosslinked agarose or crosslinked dextran, such as the CNBr-activated Sepharose 4B commercially available from Pharmacia.

[0050] The antibodies purified by differential salting-out is dissolved in a “binding buffer” and applied onto the antigen matrix, so that the immuno-complexes of the immobilized antigen and the yolk antibodies are formed. Any buffer system inert to the antigen-antibody interaction and effective to maintain the desired binding condition is useful in the present invention. Preferably, the binding buffer is selected from the group consisting of a phosphate buffer, an MES (2-[N-morpholino]ethanesulfonic acid) buffer and a bis-Tris buffer, among which an MES buffer at a concentration of 20 mM is the most preferred.

[0051] Preferably, the immunoaffinity purification is conducted in an environment of weak acid and low ionic strength, i.e., at pH within a range of about 4 to about 7 and under an ionic strength of lower than about 50 mM, e.g., less than the ionic strength of a 50 mM NaCl solution. More preferably, the antibodies were allowed to interact with the immobilized antigen at pH within a range of about 5 to about 6 and most preferably within a range of about 5.6 to about 5.8. The yolk antibodies can be dissociated from the antigen matrix by a chaotropic salt, or at a pH of lower than about 4 or higher than about 8. The activity of the collected antibodies can be restored by, for example, extensive dialysis against a low-ionic strength, non-chaotrope-containing, weakly acidic buffer.

[0052] The IgY(ΔFc) purified according the process of the invention neither activate the complement system nor binds to rheumatoid factor of mammalian sera. The immunological cross-reactivity between IgY(ΔFc) and the mammalian IgG is not significant. Thus, the invention also provide a new type of antibody suitable for clinical and research uses.

[0053] The invention also provides a broad variety of clinical and research uses of the IgY antibody prepared according to the invention.

[0054] For example, the present invention provides a pharmaceutical composition for treating or prophylaxis an animal (which includes domestic fowls, livestock and companion animals) or human patient comprising a therapeutic amount of the IgY antibody of the present invention for protecting or prophylaxis them from various etiological agents, including microorganisms, such as bacteria, native, recombinant or peptide-synthetic viruses, fungi, protozoa, nematodes and the like, and proteinaceous or non-proteinaceous substances, such as native, recombinant or peptide-synthetic allergens, toxins, venoms, hormones or any other immunogen capable of eliciting an immune response. Preferably, the purified IgY antibody is applied in combination with a pharmaceutically acceptable carrier such as water, saline and the like. The pharmaceutical composition can be delivered by ways comprising oral delivery, injection, external administration, and immunizing treatment.

[0055] The IgY antibody of the present invention is also useful for detecting an etiological agent of interest, including, for example, a pathogenic or non-pathogenic organism, such as Escherichia coli, Salmonella enterititis, and other bacterial organisms; a native, recombinant or peptide-synthetic hormone such as estrogen, progesterone, thyroxin and the like; a major histocompatibility complex antigen and the like; a native, recombinant or peptide-synthetic tumor marker such as alpha-fetoprotein, prostate specific antigen and the like; a disease state marker such as C-reactive protein, ferritin and the like; an accumulation or a residual of foreign materials such as drugs of Theophylline and digoxin; in a body sample such as a fluid, tissue, cell extract and the like, that is derived from the human or animal. In order to obtain antibodies only specific to the etiological agents, the etiological agent can be injected into the ducks as antigens for inducing the production of desired antibodies, and wherein the antigens comprise naturally purified antigens, recombinant antigens, peptide-synthetic antigens, and plasmid DNA. Using the IgY antibody obtained according to this invention, an etiological agent of interest can be quantitatively or qualitatively detected by any conventional method known in the art, such as the Ouchterlony methods (MO), the single radial immuno diffusion method (SRID), the immuno electrophoresis method (IEP), the radioimmuno assay method (RIA), the enzyme-linked immuno sorbent assay method (ELISA), the Western blot method (WB), the turbidimetric immunoassay method (TIA), the particle-enhanced turbidimetric immunoassay method, an enzymatic immunoassay, a nephelometric immunoassay, a chemiluminescent immunoassay, an immuno gold assay, or an immuno-chromatography assay.

[0056] The IgY antibody of the present invention is also adapted for use in biochips and biosensors.

[0057] The following Examples are given for the purpose of illustration only and are not intended to limit the scope of the present invention.

Example 1 Immunization Procedure for Stimulation of Specific Antibody Production

[0058] Twelve, 16-week old, domestic ducks (Anas platyrhynchos var. domestica) were individually housed for antibody and egg production. The ducks received an initial subcutaneous injection of 1-5 mg/ml of human C-reactive protein (CRP; purified from human ascites) in phosphate buffer, pH 7.5 emulsified with an equal volume of complete Freund's adjuvant. The concentration of the antigen used was generally in the range of 1 to 5 mg/ml. After the initial injection, young hens received three additional injections of 1-5 mg of antigen every two weeks. One week later, eggs began to be collected, labeled and stored at 4° C. until processed for extraction and purification of antibody. The booster procedure was repeated every four weeks during the experiment. Blood was sampled at the seventh day after each booster injection. Each blood sample was centrifuged and the resulting serum was collected.

Example 2 Extraction of Antibodies from Duck Yolks

[0059] The yolks collected from the eggs laid by the hyperimmunized ducks of Example 1 were thoroughly washed by a weak jet of distilled water, to thereby remove albumen. The volume of yolk was measured and then mixed thoroughly with distilled water in an amount of ten times the measured amount of yolk. The mixture was then held for at least two hours under 4° C., and subsequently centrifuged at 10,000 rpm in a Hitachi CR-22F centrifuge for one hour. A pale supernatant layer and a semi-solid pliable layer were formed in centrifuge tubes.

Example 3 Treatment with Absorbents

[0060] To the crude extract prepared in Example 2 were added with one of the absorbents: 2% (w/v) fumed silica (purchased from Sigma), 3% (w/v) silica dioxide (sigma), 3% (w/v) Celite diatomite (purchased from Celite Corporation), and 3 or 5% (w/v) Celite diatomite hyflo-Cel (Celite Corporation). The resultant suspensions were incubated at 4° C. for 60 minutes with gentle stirring. After completion of the incubation, the absorbents were precipitated at 4° C. at 20,000 rpm in a Hitachi CR-22F centrifuge, and the supernatants and pellets were harvested separately. Ten μl samples taken from each supernatant were subjected to non-reducing sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE).

[0061] As shown in FIG. 1, in terms of the quantity of the antibodies adsorbed by the absorbents, fumed silica has the best adsorptive activity and almost no antibody was left in the flow through solution.

[0062] Silica dioxide displays a slightly weaker affinity to immunoglobulins, which perhaps results from its lower porosity (and thus comprising a less extensive surface area) than fumed silica. On the other hand, less than 10% of the yolk antibodies were captured by either type of the diatomaceous earths.

Example 4 Differential Salting-out of Yolk Antibodies

[0063] The fumed silica pellet obtained in Example 3 was treated with 2.5 M sodium thiocyanate (pH 7.5) to elute the antibodies bound thereon. The resultant eluate was firstly precipitated with ammonium sulfate at a concentration of about 21% (w/v) based on the volume of the eluate, followed by a second precipitation with addition of ammonium sulfate to about 31% (w/v). The precipitated antibody products were re-dissolved in phosphate buffer saline (PBS). Analytical SDS-PAGE was performed on a 8% non-reducing acrylamide gel, in which 2237 μg of the crude extract of example 2 (lane 1), 10 μl of the flow through harvested in Example 3 (lane 2), 1122.25 μg of the eluate from the fumed silica pellet (lane 3), and 153 μg and 372.85 μg of the antibody products obtained in the first and second precipitation steps (lane 4 and lane 5, respectively) were loaded. The result is shown in FIG. 2. The percentage recovery and purity were determined by scanning densitometry of the gel and summarized in Table 1. TABLE 1 IgY (7.8 S) IgY (7.8 S) IgY (ΔFc) IgY (ΔFc) Total protein percentage yield/egg percentage yield/egg Crude extract 447.4 mg 4.43% 19.82 mg 26.79% 119.86 mg  Eluate 224.45 mg  8.15% 18.29 mg 41.65% 93.48 mg 1^(St) precipitation by 30.65 mg 37.82%  11.59 mg 62.18% 19.06 mg 21% (NH₄)₂SO₄ 2^(nd) precipitation by 74.57 mg 2.03%  1.51 mg 96.62% 72.05 mg 31% (NH₄)₂SO₄

[0064] As illustrated in Table 1, the resulting IgY(ΔFc) antibodies are recovered in about 76% yield (72.05 mg/l 19.86 mg×100%) in greater than 96% purity. More importantly, this purification scheme advantageously leads to the essential separation of the desired IgY(ΔFc) antibodies from the whole population of yolk antibodies constituted mainly by both IgY (7.8 S) and IgY(ΔFc) (5.7 S). In the above example, the ratio of 5.7 S antibody to 7.8 S antibody is at least 40 (i.e., 47.7).

Example 5 Partially Purified IgY(ΔFc) with Celite Diatomite

[0065] Taking advantage of the ability of diatomaceous earth to attract lipids and repulse antibodies, the crude extract prepared in Example 2 was poured onto a filtration column packed with 10% by weight of Celite diatomite based on the poured volume of the extract. The solution flowing through the column was harvested and subjected a first precipitation with 21% (w/v) ammonium sulfate based on the volume of the flow through solution. The precipitated antibodies were collected and the supernatant was divided into two parts. One part of the supernatant was precipitated with ammonium sulfate at a concentration of about 31% (w/v), while the other part was precipitated with 16% (w/v) sodium sulfate. The precipitated antibody products were re-dissolved in PBS. Analytical SDS-PAGE was performed on a 8% non-reducing acrylamide gel, in which 2012.5 μg of the crude extract of Example 2 (lane 1), 1678 μg of the flow through harvested by Celite diatomite filtration (lane 2), 94.9 μg of the eluate obtained in the first precipitation step (lane 3), and 169.65 μg and 357.75 μg of the antibody products obtained in the second precipitation step by 31% ammonium sulfate and 16% sodium sulfate (lanes 4-5) were loaded. The result is shown in FIG. 3. The percentage recovery and purity were determined by scanning densitometry of the gel and summarized in Table 2. TABLE 2 Total IgY IgY (ΔFc) IgY (ΔFc) protein percentage IgY yield/egg percentage yield/egg Crude extract 405.2 mg 11.60%  46.98 mg 29.01%   117 mg CLT filtrate 335.6 mg 5.08% 17.05 mg 30.47% 102.25 mg  1^(St) precipitation by 21% 18.98 mg 62.60%  11.88 mg 37.40%  7.10 mg (NH₄)₂SO₄ 2^(nd) precipitation by 16% 33.93 mg 6.29%  2.13 mg 77.14% 26.17 mg Na₂SO₄ 2^(nd) precipitation by 31% 71.55 mg 8.79%  6.29 mg 68.68% 49.14 mg (NH₄)₂ SO₄

[0066] As illustrated in Table 2, the resulting IgY(ΔFc) antibodies are recovered in about 77% (when sodium sulfate is used in the second precipitation step) and 69% purity (when ammonium sulfate is used in the second precipitation step), respectively, with high yields.

Example 6 Immunoaffinity Purification of Yolk Antibodies

[0067] A C-reactive protein (CRP) solution was prepared in 0.1 M carbonate buffer, pH 8.5 at a concentration of 5 mg/ml. CNBr-activated Sepharose 4B purchased from Pharmacia was washed initially with 1 mM cold HCl in an amount of ten times the matrix volume and allowed to react with the CRP solution in an amount of two times the matrix volume of at 4° C. overnight. The antigen matrix was suspended in a solution of 0.5 M ethanolamine in 20 mM Tris-HCl (pH 8.5) in a ratio of 1:1 (v/v) for 2 hours at 4° C. to block remaining protein-reactive sites. The antigen matrix was then washed with PBS containing 0.02% sodium azide and stored at 4° C.

[0068] The duck antibodies precipitated with 21% (w/v) ammonium sulfate in Example 4 and the antigen matrix prepared above were used. One ml of the antigen matrix was packed into a conventional column and soaked in 20 mM of MES (2-[N-morpholino] ethanesulfonic acid) buffer (pH 5.8). The antigen matrix was allowed to react with 0.25 ml of the antibodies formulated in the same binding buffer. The antigen matrix was washed with the binding buffer until the effluent was substantially free of protein. Bound antibodies were eluted immediately with 6 M guanidine-HCl, and the optical density thereof was measured at 280 nm after a complete dialysis. The SDS-PAGE analysis shown in FIG. 4 indicates that the affinity-purified antibodies are constituted mainly by IgY(ΔFc) antibody which is represented by a single band on the gel.

[0069] All patents and literature references cited in the present specification are hereby incorporated by reference in their entirety. In case of conflict, the present description, including definitions, will prevail.

[0070] While embodiments of the present invention have been illustrated and described, various modifications and improvements can be made by persons skilled in the art. The embodiments of the present invention are therefore described in an illustrative but not restrictive sense. It is intended that the present invention is not limited to the particular forms as illustrated, and that all the modifications not departing from the spirit and scope of the present invention are within the scope as defined in the appended claims. 

What is claimed is:
 1. A process for selectively isolating IgY antibodies from egg yolk of an anseriform bird, comprising: (a) absorbing yolk antibodies in a water-miscible fraction obtained from the egg yolk of an anseriform bird with a water insoluble non-charged absorbent selected from the group consisting of silicate, silicon compounds, carbonate, sulfate, phosphate, carbon, cellulose and synthetic fiber, ceramics, and metal oxide, and wherein the water insoluble non-charged absorbent is at an amount effective for separating the yolk antibodies from the water-miscible fraction; and (b) flowing the water insoluble non-charged absorbent with a buffer to obtain an aqueous fraction containing the yolk antibodies, wherein the IgY antibodies comprise antibodies with Fe regions and antibodies that lack Fe regions.
 2. The process of claim 1, wherein the water insoluble non-charged absorbent is a silicate selected from the group consisting of synthetic or natural clays, kaolin, talc, and calcium silicate.
 3. The process of claim 1, wherein the water insoluble non-charged absorbent is a silicon compound selected from the group consisting of fumed silica, amorphous silica, silica dioxide, silica gel, silicates, diatomaceous earth, and Fuller's earth.
 4. The process of claim 1, wherein the water insoluble non-charged absorbent is comprised of calcium carbonate or barium carbonate.
 5. The process of claim 1, wherein the water insoluble non-charged absorbent is comprised of calcium sulfate.
 6. The process of claim 1, wherein the water insoluble non-charged absorbent is comprised of calcium phosphate.
 7. The process of claim 1, wherein the water insoluble non-charged absorbent is comprised of activated carbon or carbon fiber.
 8. The process of claim 1, wherein the water insoluble non-charged absorbent is comprised of cellulose powder.
 9. The process of claim 1, wherein the water insoluble non-charged absorbent is comprised of a porous ceramic.
 10. The process of claim 1, wherein the water insoluble non-charged absorbent is comprised of aluminum oxide or titanium oxide.
 11. The process of claim 1, wherein the anseriform bird is a duck or a goose.
 12. A method for isolating avian antibodies from egg yolk, the method comprising: (a) contacting a preparation that comprises avian antibodies with a water insoluble absorbent that absorbs both avian antibodies and lipid; and (b) eluting the avian antibodies from the water insoluble absorbent with an aqueous buffer that releases the absorbed avian antibodies, but not the lipid, thereby providing an isolated preparation of avian antibodies.
 13. The process of claim 1, wherein the buffer for flowing the water insoluble non-charged absorbent in step (b) comprises a chaotropic salt.
 14. The process of claim 13, wherein the chaotropic salt comprises about 3M to about 6M guandine-HCl or about 1 M to about 3 M sodium thiocyanate.
 15. The process of claim 1, further comprising a purification step by an immunoaffinity chromatography at a pH value ranging from about 4 to about 7 under an ionic strength of lower than about 50 mM.
 16. The process of claim 15, wherein the pH value is ranging from about 5 to about
 6. 17. The process of claim 16, wherein the pH value is ranging from about 5.6 to about 5.8.
 18. The process of claim 1, wherein the aqueous fraction containing the yolk antibodies in step (b) is a flow-through solution which has flowed through the water insoluble non-charged absorbent.
 19. The process of claim 1, wherein the aqueous fraction containing the yolk antibodies in step (b) is an eluate eluted from the water insoluble non-charged absorbent.
 20. A process for selectively isolating IgY antibodies from egg yolk of an anseriform bird comprising performing first salting out by salting out an aqueous fraction containing yolk antibodies with (NH₄)₂SO₄ of a first concentration ranging from about 15% (w/v) to about 24% (w/v) based on the volume of the aqueous fraction, and then performing second salting out by salting out the aqueous fraction containing yolk antibodies treated in the first salting out with (NH₄)₂SO₄ of a second concentration ranging from about 25% (w/v) to about 40% (w/v) based on the volume of the aqueous fraction treated in the first salting out; wherein the IgY antibodies comprise antibodies with Fe regions and antibodies that lack Fc regions.
 21. The process of claim 20, wherein the first concentration is not more than about 21% (w/v) based on the volume of the aqueous fraction.
 22. The process of claim 20, wherein the second concentration is not more than about 31% (w/v) based on the volume of the aqueous fraction treated in the first salting out.
 23. The process of claim 20, wherein the anseriform bird is a duck or a goose.
 24. A method for enriching 5.7 S isoform avian antibodies relative to 7.8 S isoform avian antibodies, the method comprising: (a) precipitating 7.8 S isoform antibodies using a precipitant salt at an ionic strength less than the ionic strength of 24% (NH₄)₂SO₄ (w/v) to provide a supernatant that includes 5.7 S antibodies; and (b) precipitating the 5.7 S isoform antibodies from the supernatant using a precipitant salt, to thereby provide an isolated preparation enriched for 5.7 S isoform antibodies.
 25. The process of claim 20, further comprising a purification step by an immunoaffinity chromatography at a pH value ranging from about 4 to about 7 under an ionic strength of lower than about 50 mM.
 26. The process of claim 25, wherein the pH value is ranging from about 5 to about
 6. 27. The process of claim 26, wherein the pH value is ranging from about 5.6 to about 5.8.
 28. A process for selectively isolating IgY antibodies from egg yolk of an anseriform bird comprising: (a) absorbing yolk antibodies in a water-miscible fraction obtained from the egg yolk of an anseriform bird with a water insoluble non-charged absorbent selected from the group consisting of silicate, silicon compounds, carbonate, sulfate, phosphate, carbon, cellulose and synthetic fiber, ceramics, and metal oxide, and wherein the water insoluble non-charged absorbent is at an amount effective for separating the yolk antibodies from the water-miscible fraction; (b) flowing the water insoluble non-charged absorbent with a buffer to obtain an aqueous fraction containing the yolk antibodies; (c) salting out the aqueous fraction containing yolk antibodies in step (b) with (NH₄)₂SO₄ of a first concentration ranging from about 15% (w/v) to about 24% (w/v) based on the volume of the aqueous fraction; and (d) salting out the aqueous fraction containing yolk antibodies treated in step (c) with (NH₄)₂SO₄ of a second concentration ranging from about 25% (w/v) to about 40% (w/v) based on the volume of the aqueous fraction treated in step (c); and wherein the IgY antibodies comprise antibodies with Fc regions and antibodies lack of Fe regions.
 29. The process of claim 28, wherein the silicate comprises synthetic or natural clays, kaolin, talc, and calcium silicate.
 30. The process of claim 28, wherein the silicon compound comprises fumed silica, amorphous silica, silica dioxide, silica gel, silicates, diatomaceous earth, and Fuller's earth.
 31. The process of claim 28, wherein the carbonate comprises calcium carbonate and barium carbonate.
 32. The process of claim 28, wherein the sulfate comprises calcium sulfate.
 33. The process of claim 28, wherein the phosphate comprises calcium phosphate.
 34. The process of claim 28, wherein the carbon comprises activated carbon and carbon fiber.
 35. The process of claim 28, wherein the cellulose and synthetic fiber comprise cellulose powder.
 36. The process of claim 28, wherein the ceramics comprises porosity ceramics.
 37. The process of claim 28, wherein the metal oxide comprises aluminum oxide and titanium oxide.
 38. The process of claim 28, wherein the anseriform bird is a duck or a goose.
 39. The method of claim 12, further comprising separating 5.7 S isoform antibodies in the isolated preparation of avian antibodies from 7.8 S isoform antibodies.
 40. The process of claim 28, wherein the buffer for flowing the water insoluble non-charged absorbent in step (b) comprises a chaotropic salt.
 41. The process of claim 40, wherein the chaotropic salt comprises about 3M to about 6M guandine-HCl or about 1 M to about 3 M sodium thiocyanate.
 42. The process of claim 28, wherein the first concentration is not more than about 21% (w/v) based on the volume of the aqueous fraction.
 43. The process of claim 28, wherein the second concentration is not more than about 31% (w/v) based on the volume of the aqueous fraction treated in the first salting out.
 44. The process of claim 28, further comprising a purification step by an immunoaffinity chromatography at a pH value ranging from about 4 to about 7 under an ionic strength of lower than about 50 mM.
 45. The process of claim 44, wherein the pH value is ranging from about 5 to about
 6. 46. The process of claim 45, wherein the pH value is ranging from about 5.6 to about 5.8.
 47. The process of claim 28, wherein the aqueous fraction containing the yolk antibodies in step (b) is a flow-through solution which has flowed through the water insoluble non-charged absorbent.
 48. The process of claim 28, wherein the aqueous fraction containing the yolk antibodies in step (b) is an eluate eluted from the water insoluble non-charged absorbent.
 49. An IgY antibody selectively isolated from egg yolk of an anseriform bird, the IgY antibody being prepared according a process comprising: (a) absorbing yolk antibodies in a water-miscible fraction obtained from the egg yolk of an anseriform bird with a water insoluble non-charged absorbent selected from the group consisting of silicate, silicon compounds, carbonate, sulfate, phosphate, carbon, cellulose and synthetic fiber, ceramics, and metal oxide, and wherein the water insoluble non-charged absorbent is at an amount effective for separating the yolk antibodies from the water-miscible fraction; (b) flowing the water insoluble non-charged absorbent with a buffer to obtain an aqueous fraction containing the yolk antibodies; (c) salting out the aqueous fraction containing yolk antibodies in step (b) with (NH₄)₂SO₄ of a first concentration ranging from about 15% (w/v) to about 24% (w/v) based on the volume of the aqueous fraction; and (d) salting out the aqueous fraction containing yolk antibodies treated in step (c) with (NH₄)₂SO₄ of a second concentration ranging from about 25% (w/v) to about 40% (w/v) based on the volume of the aqueous fraction treated in step (c); and wherein the IgY antibodies comprise antibodies with Fc regions and antibodies lack of Fc regions.
 50. A preparation comprising 5.7 S isoform avian antibodies, wherein the 5.7 S are present at a concentration at least 10 fold greater than any 7.8 S isoform antibodies, if present, the preparation being prepared by a method comprising: (a) contacting a preparation that comprises avian antibodies with a water insoluble absorbent that absorbs both avian antibodies and lipid; (b) eluting avian antibodies from the water insoluble absorbent with an aqueous buffer that releases the absorbed antibodies, but not the lipid, thereby providing an eluate; and (c) separating 5.7S isoform antibodies from the eluate, the separating being preferential for 5.7 S isoform antibodies relative to 7.8 S isoform antibodies.
 51. The IgY antibody of claim 49, wherein the silicon compound comprises fumed silica, amorphous silica, silica dioxide, silica gel, silicates, diatomaceous earth, and Fuller's earth.
 52. The IgY antibody of claim 49, wherein the carbonate comprises calcium carbonate and barium carbonate.
 53. The IgY antibody of claim 49, wherein the sulfate comprises calcium sulfate.
 54. The IgY antibody of claim 49, wherein the phosphate comprises calcium phosphate.
 55. The IgY antibody of claim 49, wherein the carbon comprises activated carbon and carbon fiber.
 56. The IgY antibody of claim 49, wherein the cellulose and synthetic fiber comprise cellulose powder.
 57. The IgY antibody of claim 49, wherein the ceramics comprises porosity ceramics.
 58. The IgY antibody of claim 49, wherein the metal oxide comprises aluminum oxide and titanium oxide.
 59. The IgY antibody of claim 49, wherein the anseriform bird is a duck or a goose.
 60. The IgY antibody of claim 49, wherein the buffer for flowing the water insoluble non-charged absorbent in step (b) comprises a chaotropic salt.
 61. The IgY antibody of claim 60, wherein the chaotropic salt comprises about 3M to about 6M guandine-HCl or about 1 M to about 3 M sodium thiocyanate.
 62. The IgY antibody of claim 49, wherein the first concentration is not more than about 21% (w/v) based on the volume of the aqueous fraction.
 63. A preparation comprising 5.7 S isoform avian antibodies, wherein the 5.7 S isoform avian antibodies are at least 80% pure relative to other protein species and are present at a concentration at least 10 fold greater than any 7.8 S isoform antibodies, if present.
 64. A pharmaceutical composition comprising an IgY antibody according to claim 49 together with a pharmaceutically acceptable carrier.
 65. A kit for immunoassay, comprising an IgY antibody according to claim 49 and instructions for use. 